Non-coding RNAs in acute ischemic stroke:from brain to periphery

Acute ischemic stroke is a clinical emergency and a condition with high morbidity,mortality,and disability.Accurate predictive,diagnostic,and prognostic biomarkers and effective therapeutic targets for acute ischemic stroke remain undetermined.With innovations in high-throughput gene sequencing analysis,many aberrantly expressed non-coding RNAs(ncRNAs)in the brain and peripheral blood after acute ischemic stroke have been found in clinical samples and experimental models.Differentially expressed ncRNAs in the post-stroke brain were demonstrated to play vital roles in pathological processes,leading to neuroprotection or deterioration,thus ncRNAs can serve as therapeutic targets in acute ischemic stroke.Moreover,distinctly expressed ncRNAs in the peripheral blood can be used as biomarkers for acute ischemic stroke prediction,diagnosis,and prognosis.In particular,ncRNAs in peripheral immune cells were recently shown to be involved in the peripheral and brain immune response after acute ischemic stroke.In this review,we consolidate the latest progress of research into the roles of ncRNAs(microRNAs,long ncRNAs,and circular RNAs)in the pathological processes of acute ischemic stroke–induced brain damage,as well as the potential of these ncRNAs to act as biomarkers for acute ischemic stroke prediction,diagnosis,and prognosis.Findings from this review will provide novel ideas for the clinical application of ncRNAs in acute ischemic stroke.

非编码RNA在肺纤维化过程中的调控作用

背景:截至目前,肺纤维化的发病机制不明,治疗手段或者药物有限。大量研究发现,非编码RNA在肺纤维化的发生发展过程中发挥重要作用。目的:综述近年来非编码RNA在肺纤维化发病机制中的调控作用,深入了解肺纤维化的发病机制。方法:由第一作者应用计算机检索2000-2024年出版的文献,以“非编码RNA,微小RNA,长链非编码RNA,环状RNA,肺纤维化,综述”等为中文检索词检索中国知网、万方和维普数据库;以“ncRNA,miRNA,lncRNA,circRNA,Pulmonary fibrosis,review”等为英文检索词检索PubMed数据库,按照入选标准最终共纳入65篇文献进行综述。结果与结论:肺纤维化作为一种慢性且通常致命的肺部疾病,不仅可能自发产生,也可能是其他疾病的继发结果,主要特点是肺部间质中细胞外基质的异常增生和大量积累。非编码RNA是指由基因组转录出来的RNA分子,这些RNA分子并不涉及蛋白质的编码过程,凭借其调节能力已成为各种生物学现象中的一线分子参与者之一。非编码RNA在肺纤维化的发病机制中扮演着关键角色,微小RNA(miRNA)、长链非编码RNA(lncRNA)和环状RNA(circRNA)可以通过影响基因表达、转录后修饰以及细胞间的信号传导,参与到肺纤维化的发展过程中,为后续探索肺纤维化疾病的具体分子发生机制提供了新方向,为研发肺纤维化疾病的新靶向药物提供了理论依据及新思路。

Long noncoding RNA steroid receptor RNA activator 1 inhibits proliferation and glycolysis of esophageal squamous cell carcinoma

BACKGROUND The clinical effects and detailed roles of long non-coding RNA(LncRNA)steroid receptor RNA activator 1(SRA1)in esophageal squamous cell carcinoma(ESCC)remain ambiguous.In the present study,the complementary sites between lncRNA SRA1,miRNA-363-5p,and phospholysine phosphohistidine inorganic pyrophosphate phosphatase(LHPP)predicted via bioinformatics analysis stimulated us to hypothesize that miRNA-363-5p/LHPP axis might be required for SRA1-mediated ESCC progression.AIM To investigate the molecular events of SRA1 in the malignant behavior in ESCC.METHODS Thirty-eight ESCC tissues and paired adjacent normal tissues were acquired.SRA1 expression was detected in ESCC tissues and cell lines using quantitative reverse transcription-polymerase chain reaction.Cell counting Kit-8 assay,transwell invasion assay,glycolysis assay,and xenograft tumor model were performed to address the malignant biological behaviors of ESCC cells after the introduction of SRA1.The t-test and theχ2 test were used for comparison between groups.Survival curve analysis was performed using the Kaplan-Meier method.RESULTS SRA1 downregulation was identified in ESCC.ESCC patients exhibiting a low SRA1 expression faced shorter overall survival than those with a high SRA1 expression.The introduction of SRA1 inhibited cell proliferation,glucose uptake,and lactate production in ESCC.In vivo,the growth of ESCC was hindered by SRA1 overexpression.Then,SRA1 overexpresses the LHPP by inhibiting miRNA-363-5p.Lastly,the introduction of small interfering RNA si-LHPP or miRNA-363-5p mimic could abrogate the inhibition roles triggered by SRA1.CONCLUSION SRA1 inhibits the oncogenicity of ESCC via miRNA-363-5p/LHPP axis.The SRA1/miRNA-363-5p/LHPP pathway may be a therapeutic target for ESCC.

长链非编码RNA LINC00926调控微小RNA-331-3p对前列腺癌细胞增殖和迁移的影响

目的:探讨长链非编码RNA(lncRNA)LINC00926对前列腺癌细胞增殖和迁移的影响及分子机制。方法:前列腺癌组织和癌旁组织LINC00926表达用LncRNADisease数据库分析。采用RT-qPCR检测正常前列腺上皮RWPE-1细胞和前列腺癌细胞株22Rv1、PC3、C4-2B、LNCaP、DU-145中LINC00926的表达。选取LINC00926表达最高的前列腺癌DU-145细胞,分别转染LINC00926小干扰RNA(si-LINC00926组)和阴性对照RNA(si-NC组)。采用CCK-8法、划痕实验检测DU-145细胞增殖和迁移能力。双荧光素酶报告基因实验检测LINC00926与miR-331-3p的靶向结合。采用RT-qPCR检测DU-145细胞中miR-331-3p表达。采用Western blot检测Wnt/β-连环蛋白(β-catenin)信号通路相关蛋白表达。结果:前列腺癌组织LINC00926表达水平高于癌旁组织(P<0.05)。与RWPE-1细胞比较,LINC00926在前列腺癌22Rv1、PC3、DU-145、C4-2B、LNCaP细胞中表达水平升高,且DU-145细胞表达最高(均P<0.05)。si-NC组LINC00926表达水平高于si-LINC00926组(P<0.05)。于24、48、72、96 h,si-LINC00926组DU-145细胞增殖能力低于si-NC组(均P<0.05)。与si-NC组比较,si-LINC00926组DU-145细胞迁移能力下降(P<0.05)。LINC00926-WT和miR-331-3p共转染荧光素酶相对活性低于LINC00926-WT和miR-NC共转染(P<0.05)。si-NC组miR-331-3p表达水平低于si-LINC00926组(P<0.05)。与si-NC组比较,si-LINC00926组DU-145细胞中β-连环蛋白(β-catenin)、细胞髓细胞瘤病毒癌基因同源物蛋白(c-myc)、细胞周期蛋白D1(Cyclin D1)、周期蛋白依赖激酶3(CDK3)、B淋巴细胞瘤-2(Bcl-2)蛋白表达水平降低(均P<0.05)。结论:LINC00926在前列腺癌组织和细胞中高表达,下调LINC00926可能通过靶向miR-331-3p抑制前列腺癌细胞的增殖和迁移能力。

KRT18与mRNA及长链非编码RNA互作调控椎间盘髓核细胞损伤的机制

背景:椎间盘中差异表达的RNA结合蛋白在椎间盘退变中发挥着关键作用,其中RNA结合蛋白KRT18水平的降低与椎间盘退行性病变相关,但其在椎间盘髓核细胞中的具体作用尚未完全确定。目的:探讨KRT18与mRNA及长链非编码RNA结合互作对椎间盘髓核细胞的影响及机制。方法:对因腰部骨折或椎间盘退行性病变而接受椎间融合术的患者进行人体髓核组织取样获得正常髓核细胞和退变髓核细胞,并进行iRIP-seq、功能富集分析以及DNA微阵列分析,随后根据分析结果在髓核细胞中敲低KRT18,通过蛋白免疫印迹及qRt-PCR在蛋白和RNA水平检测相关基因水平的表达。结果与结论:通过iRIP-seq分析发现GUAAUC和AGCCUC序列中存在大量的KRT18结合位点,表明KRT18可参与调控RNA的转录、翻译、稳定性或在细胞信号传导途径中发挥作用。其能够与成熟的mRNA稳定结合,其中表达较高的基因包括CRLF1及IGFBP4等,同时与其结合的长链非编码RNA的峰值基因包括SNHG25、SNHG12、NEAT1、USP32、EIF4A2和CDH4,这些基因多涉及细胞凋亡、炎症等多种生物过程,并且能介导细胞外基质代谢的相关通路,KRT18能够调控它们的稳定性、转运、翻译、剪接等多个方面的功能,进而影响基因的表达和细胞功能。实验结果验证了在髓核细胞中敲低KRT18,细胞外基质代谢水平被抑制出现失衡,导致体外椎间盘退变。该研究首次从KRT18与mRNA及长链非编码RNA结合的角度探讨其调控机制,并推测了KRT18在椎间盘退变发病机制中的潜在功能,为今后KRT18关键功能的研究奠定了基础。

不稳定型心绞痛患者血清长链非编码RNA OIP5-AS1和微小RNA-137水平与心功能及心血管不良事件的相关性分析

目的探讨不稳定型心绞痛(UA)患者血清长链非编码RNA(lncRNA)OIP5-AS1和微小RNA-137(miR-137)水平与心功能及心血管不良事件的相关性。方法选取2022年5月至2023年8月海南省第二人民医院收治的102例UA患者为观察组。另选取本院同期102名体检健康者为对照组。UA患者根据随访6个月心血管不良事件发生情况分为发生组(n=35)和未发生组(n=67)。采用实时荧光定量聚合酶链反应法检测血清lncRNA OIP5-AS1、miR-137水平;利用Pearson法分析UA患者血清lncRNA OIP5-AS1与miR-137的相关性及lncRNA OIP5-AS1、miR-137与心功能指标的相关性;Logistic回归模型分析影响UA患者发生心血管不良事件的潜在因素;受试者工作特征曲线评估血清lncRNA OIP5-AS1、miR-137水平预测UA患者发生心血管不良事件的效能。结果观察组患者血清miR-137水平、左心室舒张末期内径(LVEDD)均明显高于/大于对照组,血清lncRNA OIP5-AS1、左心室射血分数(LVEF)水平均明显低于对照组(均P<0.001)。发生组患者血清miR-137水平、LVEDD均明显高于/大于未发生组,血清lncRNA OIP5-AS1、LVEF水平均明显低于未发生组(均P<0.001)。血清lncRNA OIP5-AS1与miR-137呈负相关(r=-0.555,P<0.001)。血清lncRNA OIP5-AS1与LVEDD呈负相关(r=-0.441,P<0.001),与LVEF呈正相关(r=0.479,P<0.001);血清miR-137与LVEDD呈正相关(r=0.466,P<0.001),与LVEF呈负相关(r=-0.472,P<0.001)。miR-137、LVEDD升高是影响UA患者发生心血管不良事件的风险因素,而lncRNA OIP5-AS1、LVEF水平升高是其保护因素(均P<0.05)。血清lncRNA OIP5-AS1、miR-137水平单独预测与二者联合预测UA患者发生心血管不良事件的曲线下面积分别为0.845、0.832、0.924,二者联合优于血清lncRNA OIP5-AS1(Z=2.146、P=0.032)、miR-137(Z=2.114、P=0.035)各自单独预测。结论发生心血管不良事件的UA患者血清lncRNA OIP5-AS1水平降低、miR-137水平升高,血清lncRNA OIP5-AS1、miR-137是影响UA患者发生心血管不良事件的潜在因素,且二者联合在预测UA患者发生心血管不良事件方面展现出更高的效能。

LncRNA FGD5-AS1通过miR-103a-3p/RNF38轴影响结肠癌细胞的恶性生物学行为

目的:探讨长链非编码RNA FGD5反义RNA1(LncRNA FGD5-AS1)靶向调控miR-103a-3p/环指蛋白38(RNF38)轴对结肠癌细胞恶性生物学行为的影响。方法:使用荧光定量PCR检测LncRNA FGD5-AS1、miR-103a-3p在人结肠黏膜上皮细胞和人结肠癌细胞SW480中的表达水平;通过StarBase和TargetScan数据库分析LncRNA FGD5-AS1、miR-103a-3p、RNF38之间的结合位点,使用双荧光酶报告基因检测进一步验证;将SW480细胞随机分为对照(Control)组、pcDNA-NC组、pcDNA-FGD5-AS1组、si-NC组、si-FGD5-AS1组、si-FGD5-AS1+inhibitor NC组、si-FGD5-AS1+miR-103a-3p inhibitor组,通过CCK-8、流式细胞术、Transwell试验、荧光定量PCR及Western blot法检测细胞增殖、凋亡、侵袭、FGD5-AS1、miR-103a-3p水平及RNF3蛋白表达水平。结果:与人结肠黏膜上皮细胞相比,SW480细胞中LncRNA FGD5-AS1表达水平显著降低(1.00±0.00比0.48±0.10,t=12.737,P<0.05),miR-103a-3p表达水平显著升高(1.00±0.00比1.61±0.18,t=8.301,P<0.05);LncRNA FGD5-AS1可靶向负调控miR-103a-3p表达(P<0.05);miR-103a-3p可靶向正调控RNF38表达(P<0.05);与pcDNA-NC组相比,pcDNA-FGD5-AS1组SW480细胞中FGD5-AS1水平升高(0.98±0.10比2.34±0.45,t=7.227,P<0.05),细胞凋亡率增加(8.64±1.32比16.21±2.75,t=6.079,P<0.05),而miR-103a-3p表达水平(1.01±0.12比0.42±0.07,t=10.403,P<0.05)、RNF38蛋白表达水平(0.59±0.09比0.32±0.17,t=3.438,P=0.006)、细胞增殖活性(0.63±0.09比0.34±0.06,t=6.567,P<0.05)、细胞侵袭能力(112.63±14.94比43.82±5.67,t=10.548,P<0.05)降低。si-FGD5-AS1组细胞变化趋势与pcDNA-FGD5-AS1组相反,且miR-103a-3p inhibitor可逆转si-FGD5-AS1组的变化(P<0.05)。结论:干扰LncRNA FGD5-AS1可能通过靶向上调miR-103a-3p,促进RNF38蛋白表达,从而提高结肠癌细胞增殖和侵袭能力,降低结肠癌细胞凋亡率,而上调LncRNA FGD5-AS1可抑制结肠癌细胞的恶性生物学行为。

Characterization of N6-methyladenosine long non-coding RNAs in sporadic congenital cataract and age-related cataract

AIM:To characterize the N6-methyladenosine(m6A)modification patterns in long non-coding RNAs(lncRNAs)in sporadic congenital cataract(CC)and age-related cataract(ARC).METHODS:Anterior capsule of the lens were collected from patients with CC and ARC.Methylated RNA immunoprecipitation with next-generation sequencing and RNA sequencing were performed to identify m6A-tagged lncRNAs and lncRNAs expression.Kyoto Encyclopedia of Genes and Genomes pathway enrichment analyses and Gene Ontology annotation were used to predict potential functions of the m6A-lncRNAs.RESULTS:Large amount of m6A peaks within lncRNA were identified for both CC and ARC,while the level was much higher in ARC(49870 peaks)than that in CC(18688 peaks),yet those difference between ARC in younger age group(ARC-1)and ARC in elder age group(ARC-2)was quite slight.A total of 1305 hypermethylated and 1178 hypomethylated lncRNAs,as well as 182 differential expressed lncRNAs were exhibited in ARC compared with CC.On the other hand,5893 hypermethylated and 5213 hypomethylated lncRNAs,as well as 155 significantly altered lncRNA were identified in ARC-2 compared with ARC-1.Altered lncRNAs in ARC were mainly associated with the organization and biogenesis of intracellular organelles,as well as nucleotide excision repair.CONCLUSION:Our results for the first time present an overview of the m6A methylomes of lncRNA in CC and ARC,providing a solid basis and uncovering a new insight to reveal the potential pathogenic mechanism of CC and ARC.

Long noncoding RNA protein-disulfide isomerase-associated 3 regulated high glucose-induced podocyte apoptosis in diabetic nephropathy through targeting miR-139-3p

BACKGROUND Podocyte apoptosis plays a vital role in proteinuria pathogenesis in diabetic nephropathy(DN).The regulatory relationship between long noncoding RNAs(lncRNAs)and podocyte apoptosis has recently become another research hot spot in the DN field.AIM To investigate whether lncRNA protein-disulfide isomerase-associated 3(Pdia3)could regulate podocyte apoptosis through miR-139-3p and revealed the underlying mechanism.METHODS Using normal glucose or high glucose(HG)-cultured podocytes,the cellular functions and exact mechanisms underlying the regulatory effects of lncRNA Pdia3 on podocyte apoptosis and endoplasmic reticulum stress(ERS)were explored.LncRNA Pdia3 and miR-139-3p expression were measured through quantitative real-time polymerase chain reaction.Relative cell viability was detected through the cell counting kit-8 colorimetric assay.The podocyte apoptosis rate in each group was measured through flow cytometry.The interaction between lncRNA Pdia3 and miR-139-3p was examined through the dual luciferase reporter assay.Finally,western blotting was performed to detect the effect of lncRNA Pdia3 on podocyte apoptosis and ERS via miR-139-3p.RESULTS The expression of lncRNA Pdia3 was significantly downregulated in HG-cultured podocytes.Next,lncRNA Pdia3 was involved in HG-induced podocyte apoptosis.Furthermore,the dual luciferase reporter assay confirmed the direct interaction between lncRNA Pdia3 and miR-139-3p.LncRNA Pdia3 overexpression attenuated podocyte apoptosis and ERS through miR-139-3p in HG-cultured podocytes.CONCLUSION Taken together,this study demonstrated that lncRNA Pdia3 overexpression could attenuate HG-induced podocyte apoptosis and ERS by acting as a competing endogenous RNA of miR-139-3p,which might provide a potential therapeutic target for DN.

Molecular mechanisms underlying roles of long non-coding RNA small nucleolar RNA host gene 16 in digestive system cancers

This editorial reviews the molecular mechanisms underlying the roles of the long non-coding RNA(lncRNA)small nucleolar RNA host gene 16(SNHG16)in digestive system cancers based on two recent studies on lncRNAs in digestive system tumors.The first study,by Zhao et al,explored how hBD-1 affects colon cancer,via the lncRNA TCONS_00014506,by inhibiting mTOR and promoting autophagy.The second one,by Li et al,identified the lncRNA prion protein testis specific(PRNT)as a factor in oxaliplatin resistance by sponging ZNF184 to regulate HIPK2 and influence colorectal cancer progression and chemoresistance,suggesting PRNT as a potential therapeutic target for colorectal cancer.Both of these two articles discuss the mechanisms by which lncRNAs contribute to the development and progression of digestive system cancers.As a recent research hotspot,SNHG16 is a typical lncRNA that has been extensively studied for its association with digestive system cancers.The prevailing hypothesis is that SNHG16 participates in the development and progression of digestive system tumors by acting as a competing endogenous RNA,interacting with other proteins,regulating various genes,and affecting downstream target molecules.This review systematically examines the recently reported biological functions,related molecular mechanisms,and potential clinical significance of SNHG16 in various digestive system cancers,and explores the relationship between SNHG16 and digestive system cancers.The findings suggest that SNHG16 may serve as a potential biomarker and therapeutic target for human digestive system cancers.

Novel insights on oral squamous cell carcinoma management using long non-coding RNAs

Oral squamous cell carcinoma(OSCC)is one of the most prevalent forms of head and neck squamous cell carcinomas(HNSCC)with a poor overall survival rate(about 50%),particularly in cases of metastasis.RNA-based cancer biomarkers are a relatively advanced concept,and non-coding RNAs currently have shown promising roles in the detection and treatment of various malignancies.This review underlines the function of long non-coding RNAs(lncRNAs)in the OSCC and its subsequent clinical implications.LncRNAs,a class of non-coding RNAs,are larger than 200 nucleotides and resemble mRNA in numerous ways.However,unlike mRNA,lncRNA regulates multiple druggable and non-druggable signaling molecules through simultaneous interaction with DNA,RNA,proteins,or microRNAs depending on concentration and localization in cells.Upregulation of oncogenic lncRNAs and downregulation of tumor suppressor lncRNAs are evident in OSCC tissues and body fluids such as blood and saliva indicating their potential as valuable biomarkers.Targeted inhibition of candidate oncogenic lncRNAs or overexpression of tumor suppressor lncRNAs showed potential therapeutic roles in in-vivo animal models.The types of lncRNAs that are expressed differentially in OSCC tissue and bodily fluids have been systematically documented with specificity and sensitivity.This review thoroughly discusses the biological functions of such lncRNAs in OSCC cell survival,proliferation,invasion,migration,metastasis,angiogenesis,metabolism,epigenetic modification,tumor immune microenvironment,and drug resistance.Subsequently,we addressed the diagnostic and therapeutic importance of lncRNAs in OSCC pre-clinical and clinical systems,providing details on ongoing research and outlining potential future directions for advancements in this field.In essence,this review could be a valuable resource by offering comprehensive and current insights into lncRNAs in OSCC for researchers in fundamental and clinical domains.

Long Non-coding RNA PCED1B Antisense RNA 1 Promotes Cell Proliferation and Invasion in Hepatocellular Carcinoma by Regulating the MicroRNA-34a/CD44 Axis

Objective This study aimed to examine the role of long non-coding RNA PCED1B antisense RNA 1(PCED1B-AS1)in the development of hepatocellular carcinoma(HCC).Methods A total of 62 pairs of HCC tissues and adjacent non-tumor tissues were obtained from 62 HCC patients.The interactions of PCED1B-AS1 and microRNA-34a(miR-34a)were detected by dual luciferase activity assay and RNA pull-down assay.The RNA expression levels of PCED1B-AS1,miR-34a and CD44 were detected by RT-qPCR,and the protein expression level of CD44 was determined by Western blotting.The cell proliferation was detected by cell proliferation assay,and the cell invasion and migration by transwell invasion assay.The HCC tumor growth after PCED1B-AS1 was downregulated was determined by in vivo animal study.Results PCED1B-AS1 was highly expressed in HCC tissues,which was associated with poor survival of HCC patients.Furthermore,PCED1B-AS1 interacted with miR-34a in HCC cells,but they did not regulate the expression of each other.Additionally,PCED1B-AS1 increased the expression level of CD44,which was targeted by miR-34a.The cell proliferation and invasion assay revealed that miR-34a inhibited the proliferation and invasion of HCC in vitro,while CD44 exhibited the opposite effects.Furthermore,PCED1B-AS1 suppressed the role of miR-34a.Moreover,the knockdown of PCED1B-AS1 repressed the HCC tumor growth in nude mice in vivo.Conclusion PCED1B-AS1 may play an oncogenic role by regulating the miR-34a/CD44 axis in HCC.

Role of long non-coding RNAs in non-alcoholic fatty liver disease

Non-alcoholic fatty liver disease(NAFLD)is emerging as a common cause of chronic liver disease in children and adults.NAFLD can progress to steatohepa-titis and potentially even hepatocellular carcinoma.Early identification of pati-ents at risk for progressive disease is crucial for managing NAFLD.Recent studies have identified long noncoding RNAs(lncRNAs),circular RNAs,and microRNAs as playing important roles in the pathogenesis of NAFLD.These noncoding RNAs are involved in modulating several metabolic pathways such as hepatic glucose and lipid metabolism,oxidative stress,and even carcinogenesis.Elevated levels of lncARSR and lncRNA nuclear-enriched abundant transcript 1 have been found in patients with NAFLD.In addition,lncRNAs such as PRYP4-3 and RP11-128N14.5 can distinguish patients with NAFLD from healthy indi-viduals.Increased MEG3 expression has been observed in both NAFLD and non-alcoholic steatohepatitis,suggesting that it may help predict patients at risk for disease progression.With advances in transcriptomics,we may discover additional targets to help in the identification and prognostication of NAFLD.

小细胞外囊泡及其携带的非编码RNA在非酒精性脂肪性肝病中的作用

小细胞外囊泡(small extracellular vesicles,sEVs)是由细胞分泌的一种细胞外囊泡,产生于多泡体,多泡体与质膜融合并释放到细胞外基质。由于小细胞外囊泡可以携带分子质量相对较小的核酸、蛋白质、脂质,能够执行细胞间物质传递、细胞间通讯等功能。因此,小细胞外囊泡及其携带的非编码RNA不仅参与细胞正常生理过程,也可以在多种疾病的发生发展过程中起重要作用。本文综述了小细胞外囊泡在非酒精性脂肪性肝病(NAFLD)中的作用,小细胞外囊泡及其携带的非编码RNA不仅有望成为NAFLD诊断的标志物,同时也具有治疗NAFLD的潜在作用,或能为治疗NAFLD提供新思路。

非编码RNA在颞下颌关节炎中的研究进展

颞下颌关节炎(temporomandibular joint osteoarthritis,TMJOA)是一种临床常见疾病,但发病机制尚不明确且缺乏有效的治疗手段,给患者带来很大困扰。因此,探究TMJOA的发病机制,寻找有效的治疗方法具有重要意义。近年来的研究表明,非编码RNA(noncoding RNA,ncRNA)参与调控TMJOA的发生、发展,在其诊断和治疗方面具有巨大潜力,因此有望成为新的诊断标志物和治疗靶标。本文将对ncRNA在TMJOA中的研究进展作一综述。

血清LncRNA HCG11及miR-26b-5p与急性缺血性脑卒中患者脑梗死面积及功能预后的相关性

目的研究急性缺血性脑卒中患者血清长链非编码RNA人类白细胞抗原复合物组11(long non coding RNA human leukocyte antigen complex group 11,LncRNA HCG11)及微小核糖核酸-26b-5p(microRNA-26b-5p,miR-26b-5p)水平与脑梗死面积及功能预后的相关性。方法选取2021年1月至2022年12月本院收治的急性缺血性脑卒中患者106例,根据梗死面积将其分为小面积组、中面积组和大面积组,随访1年后根据改良Rankin量表(modified Rankin Scale,mRS)分为预后良好组和预后不良组。采用qRT-PCR检测LncRNA HCG11,miR-26b-5p相对表达量;采用Logistic回归分析影响患者预后的因素;绘制受试者工作特征(receiver operating characteristic,ROC)曲线分析LncRNA HCG11和miR-26b-5p对患者梗死面积的诊断及对预后的预测价值。采用Spearman相关分析LncRNA HCG11、miR-26b-5p与梗死面积及美国国立卫生研究院卒中量表(National Institutes of Health Stroke Scale,NHISS)的相关性。结果急性缺血性脑卒中大面积梗死患者的LncRNA HCG11水平升高,miR-26b-5p水平降低(P<0.05);与预后良好患者相比,预后不良患者的LncRNA HCG11水平升高,miR-26b-5p水平降低(P<0.05);不同梗死面积患者高血压史、高血脂史以及NHISS评分、C-反应蛋白(C-reactive protein,CRP)之间比较,差异具有统计学意义(P<0.05);LncRNA HCG11与梗死面积及NHISS均呈正相关(r_(梗死面积)=0.553,P_(梗死面积)<0.001;r_(NHISS)=0.462,P_(NHISS)<0.001),miR-26b-5p与梗死面积及NHISS均呈负相关(r'_(梗死面积)=-0.534,P'_(梗死面积)<0.001;r'_(NHISS)=-0.447,P'_(NHISS)<0.001);miR-26b-5p为影响患者预后不良的保护因素,高血压史、NHISS评分、CRP和LncRNA HCG11为患者预后不良的影响因素(P<0.05);LncRNA HCG11和miR-26b-5p及联合诊断患者梗死面积优于单独指标诊断(Z_(LncRNA HCG11)=3.049,P_(LncRNA HCG11)=0.002;Z_(miR-26b-5p)=2.657,P_(miR-26b-5p)=0.008,AUC=0.937);且LncRNA HCG11+miR-26b-5p对患者预后的预测能力显著优于LncRNA HCG11、miR-26b-5p、CRP、NHISS单独指标(Z_(LncRNA HCG11)=2.207,P_(LncRNA HCG11)=0.027;Z_(miR-26b-5p)=2.080,P_(miR-26b-5p)=0.038;Z_(CRP)=2.341,P_(CRP)=0.019;Z_(NHISS)=2.093,P_(NHISS)=0.036,AUC=0.892);LncRNA HCG11与miR-26b-5p呈负相关(r=-0.425,P<0.05)。结论急性缺血性脑卒中患者血清LncRNA HCG11水平升高,miR-26b-5p水平降低,均为患者脑梗死面积及功能预后的影响因素,对患者脑梗死面积及功能预后具有一定的诊断及预测价值。

Long non-coding RNA VPS9D1-AS1对乳腺癌细胞恶性行为的影响和机制

目的探讨长链非编码RNA(LncRNA)VPS9D1-AS1对乳腺癌细胞恶性行为的影响和机制。方法收集49例接受手术的乳腺癌患者的乳腺癌组织和癌旁组织,体外培养人正常乳腺上皮细胞MCF-10A和乳腺癌细胞系MCF-7、T47D、BT549,采用实时荧光定量PCR(RT-qPCR)检测miR-4695-5p及LncRNA VPS9D1-AS1表达水平;选择MCF-7细胞分别转染si-NC、si-LncRNA VPS9D1-AS1、pcDNA、pcDNA-LncRNA VPS9D1-AS1、miR-NC、miR-4695-5p模拟物、anti-miR-NC+si-LncRNA VPS9D1-AS1、anti-miR-4695-5p+si-LncRNA VPS9D1-AS1,采用RT-qPCR检测MCF-7细胞中LncRNA VPS9D1-AS1、miR-4695-5p表达水平,CCK-8和Transwell实验评估细胞存活率和迁移侵袭数,蛋白质印记法检测IL-6、MMP2、MMP9蛋白水平;双荧光素酶实验证实LncRNA VPS9D1-AS1与miR-4695-5p的靶向关系。结果LncRNA VPS9D1-AS1在乳腺癌组织和MCF-7、T47D、BT549细胞系中表达上调(P<0.05),miR-4695-5p表达下调(P<0.05),MCF-7细胞中LncRNA VPS9D1-AS1、miR-4695-5p变化最明显,选择MCF-7细胞进行后续实验;转染LncRNA VPS9D1-AS1后,MCF-7细胞存活率、细胞迁移和侵袭数以及IL-6、MMP2、MMP9蛋白水平降低(P<0.05);转染miR-4695-5p模拟物后,miR-4695-5p表达升高(P<0.05),MCF-7细胞存活率、细胞迁移和侵袭数及IL-6、MMP2、MMP9蛋白水平降低(P<0.05);转染pcDNA-LncRNA VPS9D1-AS1后,MCF-7细胞中miR-4695-5p表达下降(P<0.05);共转染anti-miR-4695-5p+si-LncRNA VPS9D1-AS1后,MCF-7细胞存活率、迁移数和侵袭数及IL-6、MMP2、MMP9蛋白水平升高(P<0.05)。结论干扰LncRNA VPS9D1-AS1通过靶向上调miR-4695-5p抑制促炎因子IL-6表达,进而抑制乳腺癌MCF-7细胞增殖、迁移及侵袭。

长链非编码RNA LINC01370对黑色素瘤细胞增殖和侵袭的影响及机制实验研究

目的:探讨长链非编码RNA(lncRNA)LINC01370对黑色素瘤细胞增殖和侵袭的影响及其作用机制。方法:采用Cancer LncRNA Census数据库比较黑色素瘤组织和正常皮肤组织中LINC01370表达差异。RT-qPCR检测人表皮黑色素细胞HEM和黑色素瘤细胞(VMM5A、WM266-4、A2058、A-375)中LINC01370的表达水平,选取表达水平最低的细胞进行后续实验。将LINC01370高表达质粒和对照质粒转染至A2058细胞,分为LINC01370组和NC组。采用克隆形成实验检测A2058细胞增殖能力,Transwell实验检测A2058细胞能力,Western blot检测A2058细胞中增殖和侵袭蛋白表达。双荧光素酶报告基因实验验证LINC01370和miR-1246的靶向关系。采用RT-qPCR检测A2058细胞中miR-1246表达。结果:LINC01370在黑色素瘤组织中的表达水平低于正常皮肤组织(P<0.01)。LINC01370在VMM5A、WM266-4、A2058、A-375细胞中的表达水平低于HEM细胞,且A2058细胞表达水平最低(均P<0.05)。与NC组比较,LINC01370组A2058细胞LINC01370表达水平升高(P<0.01)。与NC组比较,LINC01370组A2058细胞增殖能力、侵袭细胞数以及细胞周期蛋白依赖性激酶3(Cdk3)、细胞周期蛋白C(Cyclin C)、转化生长因子-β(TGF-β)、叉头框C2(FOXC2)蛋白表达水平降低(均P<0.01)。miR-1246与LINC01370-WT质粒共转染的相对荧光素酶活性低于miR-NC与LINC01370-WT质粒共转染(P<0.01)。与NC组比较,LINC01370组A2058细胞miR-1246表达水平降低(P<0.01)。结论:LINC01370在黑色素瘤组织及细胞中低表达,LINC01370可能通过敲低miR-1246表达抑制黑色素瘤细胞的增殖和侵袭。

非编码小RNA在口腔黏膜下纤维性变中的研究进展

口腔黏膜下纤维性变(oral submucous fibrosis,OSF)是口腔黏膜最常见的癌前病变之一,其发病机制至今尚未完全阐明。非编码小RNA(small non-coding RNAs,SncRNAs)是一类不编码蛋白质的RNA分子,已被广泛报道参与多种人类疾病的调控。越来越多的研究表明多种SncRNAs在OSF发病过程中发挥重要作用。现有研究表明,微RNA(microRNAs,miRNAs)通过调控相关转录因子和基因表达或上皮间充质转化来调控成纤维细胞(fbroblasts,FB)活化而参与OSF疾病进展;长非编码RNA(long noncoding RNAs,lncRNAs)通过调控转化生长因子-β/母体抗瘫抑制因子(transforming growth factor-β/suppressor of mothers against decapentaplegic,TGF-β/Smad)信号通路或与miRNA相互作用参与OSF的发生发展;环状RNA(circular RNAs,circRNAs)通过与miRNA相互作用在OSF中发挥作用;tRNA衍生的小RNA(tRNA-derived small RNAs,tsRNAs)参与多种纤维化疾病的进展,但其在OSF中的具体作用机制仍需进一步探索。未来仍需重点关注SncRNAs介导OSF进展的作用靶点,探究其对OSF的作用功能及分子机制,以期为诊断和治疗OSF提供新思路。

生物信息分析验证基于lncRNA标签预测HPV阴性头颈部鳞状细胞癌患者总生存率

目的:采用生物信息分析方法研究影响HPV阴性头颈部鳞状细胞癌(HNSCC)患者总生存率的相关因素,为HNSCC患者的预后预测及治疗提供依据。方法:从TCGA数据库获取HPV阴性HNSCC患者的病变组织和癌旁组织的原始RNA测序数据以及相应病人的临床信息,SurvivalR工具包对所有差异表达的长链非编码RNA(lncRNA)进行单变量Cox回归分析,使用JAVA程序,利用MSigDBC2经典通路基因集集合进行基因集富集分析,采用LASSO方法的Cox回归对数据降维和模型构建,计算每个患者的风险评分。结果:研究发现153个lncRNA与HPV阴性HNSCC患者的总生存率显著相关,时间依赖性分析表明,13个lncRNA特征在训练集中具有良好的预测性能,多变量Cox回归和分层分析表明,基于13-lncRNA标签的风险评分可作为HPV阴性HNSCC患者的独立预后因素。结论:13-lncRNA标签可能是HPV阴性HNSCC预后的新型独立生物标志物。